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利用一种在链霉菌中创建和筛选随机突变文库的有效方法对芽孢形成控制蛋白SsgA进行表征。

Characterization of the sporulation control protein SsgA by use of an efficient method to create and screen random mutant libraries in streptomycetes.

作者信息

Traag Bjørn A, Seghezzi Nicolas, Vijgenboom Erik, van Wezel Gilles P

机构信息

Microbial Development, Leiden Institute of Chemistry, Leiden University, P.O. Box 9502, 2300 RA Leiden, The Netherlands.

出版信息

Appl Environ Microbiol. 2007 Apr;73(7):2085-92. doi: 10.1128/AEM.02755-06. Epub 2007 Feb 9.

Abstract

Filamentous actinomycetes are commercially widely used as producers of natural products. However, the mycelial lifestyle of actinomycetes has been a major bottleneck in their commercialization, and screening is difficult due to their poor growth on microtiter plates. We previously demonstrated that the enhanced expression of the cell division activator protein SsgA results in the fragmented growth of streptomycetes, with enhanced growth rates and improved product formation. We here describe a novel and efficient method to create, maintain, and screen mutant libraries in streptomycetes and the application of this method for the functional analysis of Streptomyces coelicolor ssgA. The variants were amplified directly from deep-frozen biomass suspensions. Around 800 ssgA variants, including single-amino-acid-substitution mutants corresponding to more than half of all SsgA residues, were analyzed for their abilities to restore sporulation to an ssgA mutant. The essential residues were clustered in three main sections, and hardly any were in the carboxy-terminal third of the protein. The majority of the crucial residues were conserved among all SsgA-like proteins (SALPs). However, the essential residues L29, D58, and S89 were conserved only in SsgA orthologues and not in other SALPs, suggesting an SsgA-specific function.

摘要

丝状放线菌作为天然产物的生产者在商业上被广泛使用。然而,放线菌的菌丝体生活方式一直是其商业化的主要瓶颈,并且由于它们在微量滴定板上生长不佳,筛选工作困难重重。我们之前证明,细胞分裂激活蛋白SsgA的表达增强会导致链霉菌呈碎片化生长,生长速率提高且产物形成得到改善。我们在此描述一种在链霉菌中创建、维持和筛选突变体文库的新颖且高效的方法,以及该方法在天蓝色链霉菌ssgA功能分析中的应用。这些变体直接从深度冷冻的生物质悬浮液中扩增得到。分析了约800个ssgA变体,包括对应于所有SsgA残基一半以上的单氨基酸取代突变体,以评估它们恢复ssgA突变体孢子形成的能力。必需残基聚集在三个主要区域,蛋白质的羧基末端三分之一几乎没有。大多数关键残基在所有SsgA样蛋白(SALP)中保守。然而,必需残基L29、D58和S89仅在SsgA直系同源物中保守,而在其他SALP中不保守,这表明存在SsgA特异性功能。

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引用本文的文献

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Open Biol. 2013 Oct 23;3(10):130073. doi: 10.1098/rsob.130073.
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